Transcript Document
Biology 177: Principles
of Modern Microscopy
Lecture 13:
Super-resolution microscopy: Part I
Lecture 13: Fluorescent labeling,
multi-sprectral imaging and FRET
• Review of previous lecture
• FRET
• FLIM
• Super resolution microscopy
• NSOM
• Scanning probe microscopy
Summary of spectral unmixing
Förster Resonance Energy Transfer
(FRET)
• Great method for the detection of:
1. Protein-protein interactions
2. Enzymatic activity
3. Small molecules inside a cell
FRET:
Resonance Energy Transfer (non-radiative)
The Good: FRET as a molecular yardstick
Transfer of energy from one dye to
another
Depends on:
Spectral overlap
Distance
Alignment
donor
acceptor
FRET:
Optimize spectral overlap
Optimize k2 -- alignment of dipoles
Minimize direct excitement of the acceptor
(extra challenge for filter design)
FRET Diagram
Non-radiative transfer
4nsec
-xxLess
0.8 emitted
-xxLess
KT = (1/τD) • [R0/r]6
The Förster Equations.
R0 = 2.11 × 10-2 • [κ2 • J(λ) • η-4 • QD]1/6
J (λ)
eA
r is the center-to-center distance (in cm) between the donor and acceptor
tD is the fluorescence lifetime of the donor in the absence of FRET
k2 is the dipole-dipole orientation factor,
QD is the quantum yield of the donor in the absence of the acceptor
is the refractive index of the intervening medium,
FD (l) is the fluorescence emission intensity at a given wavelength l (in cm)
eA (l) is the extinction coefficient of the acceptor (in cm -1 M -1).
The orientation factor k2 can vary between 0 and 4, but
typically k2 = 2/3 for randomly oriented molecules (Stryer, 1978).
When r = R0, the efficiency of FRET is 50%
(fluorescein-tetramethylrhodamine pair is 55 Å)
More about FRET (Förster Resonance Energy Transfer)
Isolated donor
Donor distance too great
Donor distance correct
Effective between 10-100 Å only
Emission and excitation spectrum must significantly overlap
Note: donor transfers non-radiatively to the acceptor
From J. Paul Robinson, Purdue University
Optimizing FRET: Designs of new FRET pairs
• Difficult to find two FRET pairs that can use in same cell
• Used as Caspase 3 biosensors and for ratiometric imaging
Properties of fluorescent protein variants
Shaner et al, Nature Biotechnology, 2004
Optimizing FRET: Designs of new FRET pairs
• mAmetrine developed
by directed protein
evolution from violet
excitable GFP variant
• Bright, extinction
coefficient = 44,800 M-1
cm-1
• Quantum yield = 0.58
• But bleaches, 42% of
mCitrine time and 1.7%
of tdTomato
Problems with FRET
4nsec
1. The acceptor excited directly by the exciting light
• “FRET” signal with no exchange
• Increased background
• Decreases effective range for FRET assay
Problems with FRET
2. Hard to really serve as a molecular yardstick*
• Orientation seldom known
assume k2 = 2/3 (random assortment)
• Exchange depends on environment of dipoles
• Amount of FRET varies with the lifetime of the
donor fluorophore
* r = R0, the efficiency of FRET is 50%
(fluorescein-tetramethylrhodamine pair is 55 Å)
Amount of FRET varies with the
lifetime of the donor fluorophore
4nsec
Longer lifetime of the donor gives longer time to
permit the energy transfer (more for longer)
Added Bonus: Allows lifetime detection to reject
direct excitement of the acceptor (FRET=late)
Fluorescence Lifetime Imaging Microscopy
(FLIM)
• Measure spatial distribution of differences in the
timing of fluorescence excitation of fluorophores
• Combines microscopy with fluorescence
spectroscopy
• Fluorescent lifetimes very short (ns) so need fast
excitation and/or fast detectors
• Requirements for FLIM instruments
1. Excitation light intensity modulated or pulsed
2. Emitted fluorescence measured time resolved
Fluorescence Lifetime Imaging Microscopy
(FLIM)
• Two methods for FLIM
1. Frequency-domain
1.
2.
Intensity of excitation light continuously modulated
For emission measure phase shift & decrease in modulation
2. Time-domain
1.
2.
Pulsed excitation that is faster than fluorescence lifetime
Emission measurement is time-resolved
FRET and FLIM
• Donor fluorescence lifetime during FRET reduced
compared to control donor fluorescence lifetime
• During FRET, donor fluorescence lifetime less than
control donor fluorescence lifetime (tD)
KT = (1/τD) • [R0/r]6
• But isn’t it easier to image decreases in donor
fluorescence intensity rather than measure
fluorescence lifetime?
FRET and FLIM
• Remember all those nonlinearities from last
lecture?
• Brightness (or intensity) of fluorophore, as
measured on your image, more than just eQ
1.
2.
3.
4.
Local concentration of fluorophore
Optical path of microscope
Local excitation light intensity
Local fluorescence detection efficiency
• FLIM provides independent measure of local donor
lifetime
Going back to those problems with FRET:
These drawbacks can all be used to make sensors
Change in FRET for changes in:
• Orientation
• cameleon dye for Ca++
• Local environment
• Phosphate near fluorophore
• Membrane voltage (flash)
• Change in lifetime of donor
• Binding of molecule displacing water
Cameleon: FRET-based and genetically-encoded calcium probe
Calmodulin bonds Ca2+
and changes its conformation
[Ca2+]
Cameleon family: calmodulin-based
indicators of [Ca2+] using FRET
Miyawaki et al, Nature, 1997
isosbestic point
Paper to read
• Pearson, H., 2007. The good, the bad and the ugly.
Nature 447, 138-140.
• http://www.nature.com/nature/journal/v447/n714
1/full/447138a.html
Spatial Resolution of Biological Imaging Techniques
• Resolution is diffraction
limited.
• Abbe (1873) reported that
smallest resolvable distance
between two points (d)
using a conventional
microscope may never be
smaller than half the
wavelength of the imaging
light (~200 nm)
Ernst Abbe (1840-1905)
Super-resolution microscopy
• Most recent Nobel
prize in Chemistry
• Many ways to achieve
• Some more super than
others.
Spatial Resolution of Biological Imaging Techniques
Super-resolution microscopy
1. “True” super-resolution techniques
• Subwavelength imaging
• Capture information in evanescent waves
• Quantum mechanical phenomenon
2. “Functional” super-resolution techniques
1. Deterministic
• Exploit nonlinear responses of fluorophores
2. Stochastic
• Exploit the complex temporal behaviors of fluorophores
Spatial Resolution of Biological Imaging Techniques
“True” super-resolution
“Functional”
Near-Field Scanning Optical Microscopy
(NSOM)
• Scanning Near-Field Optical Microscopy (SNOM)
• Likely the super-resolution technique with the
highest resolution
• But only for superficial structures
• A form of Scanning Probe Microscopy (SPM)
Scanning Tunneling Microscopy
• Images surface at
atomic level
• Developed in 1981
• Binning and Rohrer
won Nobel for its
development
Scanning Tunneling Microscopy
• Images surface at
atomic level
• Developed in 1981
• Binning and Rohrer
won Nobel for its
development
• Works via quantum
tunneling
• Schrödinger equation
Near-Field Scanning Optical Microscopy (NSOM)
Break the diffraction limit by working in the near-field
Illuminated “spot” is smaller
than diffraction limit
(about the size of the tip for a
distance equivalent to tip
diameter)
Launch light through small
aperture
Near-field = distance of a couple of
tip diameters
NSOM working in the near-field
• Aperture diameter less
than the wavelength of
light
• In 1993 Eric Betzig and
Robert Chichester used
NSOM for repetitive
single molecule imaging
NSOM working in the near-field
• Near-field near surface of
object, < λ of light
• Near-field consists of
light as evanescent wave
• Evanescent waves higher
frequency, more
information
• Evanescent waves
quantum tunneling
phenomenon
• Product of Schrödinger
wave equations
Near-Field Scanning Optical Microscopy (NSOM)
How to make an NSOM tip
Tip of pulled quartz fiber
Aluminize tip to minimize loss of
light
Very small fraction of light
makes it through small
(50nm) aperture
Near-Field Scanning Optical Microscopy (NSOM)
SEM of tip
Tip shining on sample
(can detect with wide-field)
How to move the tip? Steal from AFM
Atomic Force Microscopy (AFM)
Atomic Force Microscopy (AFM)
• Child of STM
• Invented by Gerd
Binnig, first
experiments 1986
• 1000 times better
resolution than optical
microscopes
• Scan specimen surface
with very sharp tip
AFM tips
• Most made of silicon but borosilicate glass and
silicon nitride also used
Silicon Nitride
Sharp tip
Super tip
Atomic Force Microscopy (AFM)
• Big advantage over SEM is
that can image in liquid
• Requires liquid cell for AFM
Two patches with different micelle
orientation
AFM has two types of imaging modes
Modification to do tapping or non-contact mode
AFM (tapping mode) of IgG
AFM does have some disadvantages
1. Imaging area is small
2. Scan speed slow
3. Can be affected by
nonlinearities
4. Image artifacts, e.g.
steep walls or
overhangs
Near-Field Scanning Optical Microscopy (NSOM)
Break the diffraction limit by working in the near-field
• Like AFM can do NSOM
with tapping mode
• Requires bent tip
• Move tip up and down
like AFM
• Not best way of doing
NSOM
• Hard to make probe
• Bend causes loss of light
If not tapping like AFM how else to scan tip in NSOM?
Shear force mode.
Advantage: don’t need laser to keep track of probe.
To keep tip in near-field, need to be ~50nm from surface
Sense presence of surface from dithering tip (lateral)
(Increased shear force when surface is near)
Keep dithering amplitude low <10 nm
Shear force mode with non optical feedback
• Use real-time feedback
to keep probe in nearfield range but not
touching
• Tip can be oscillated at
resonance frequency
• Tip can be straight
• Easier to make
• Cheaper
• But surface needs to be
relatively flat
NSOM instrument
NSOM tips
NSOM images
Single molecules of DiI on glass surface
NSOM images
NSOM disadvantages
• Practically zero working distance and small depth of
field.
• Extremely long scan times for high resolution images or
large specimen areas.
• Very low little light through such a tiny aperture.
• Only features at surface of specimens can be studied.
• Fiber optic probes are somewhat problematic for
imaging soft materials due to their high spring
constants, especially in shear-force mode.
Performance range of optical microscopy
SIM/STP
MRI
OCT
SPIM
Depth
(um)
CLSM
LM
NSOM
TIRF
Resolution
(um)
Homework 5
There are so many different ways to do superresolution microscopy. Interestingly, an entirely
novel method was just published this year in
Science called expansion microscopy.
Question: What makes this super-resolution
technique so novel compared to all the others?
Hint: see this figure from Ke, M.-T., Fujimoto,
S., Imai, T., 2013. Nat Neurosci 16, 1154-1161.